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定点诱变氨基酸取代对人14 kDa β-半乳糖苷结合凝集素的碳水化合物识别及稳定性的影响。

Effect of amino acid substitution by sited-directed mutagenesis on the carbohydrate recognition and stability of human 14-kDa beta-galactoside-binding lectin.

作者信息

Hirabayashi J, Kasai K

机构信息

Department of Biological Chemistry, Faculty of Pharmaceutical Sciences, Teikyo University, Kanagawa, Japan.

出版信息

J Biol Chem. 1991 Dec 15;266(35):23648-53.

PMID:1721052
Abstract

The roles of selected amino acid residues of human 14-kDa beta-galactoside-binding lectin were studied by site-directed mutagenesis. Ten mutant lectin proteins were produced, in each of which one of the residues regarded as possibly related to the stability of the lectin (6 cysteine residues) or one of those highly conserved in the vertebrate beta-galactoside-binding lectin family (Asn46, Trp68, Glu71, and Arg73), was substituted. All the mutant lectins in which one of the cysteine residues had been substituted with serine (C2S, C16S, C42S, C60S, C88S, and C130S) proved to have sugar binding ability comparable with that of the wild-type lectin. In addition, one of the mutants in which Cys2 was substituted (C2S) was found to have become considerably more stable under non-reducing conditions. It retained asialofetuin binding activity for over a week in the absence of beta-mercaptoethanol, while the wild-type lectin lost it within a day. This suggests that oxidation of Cys2 could be a key process in the inactivation of human 14-kDa lectin. Substitution of highly conservative Trp68 to tyrosine (W68Y) slightly reduced lactose binding ability, but the mutant was still adsorbed strongly on asialofetuin-agarose. Other mutant lectins in which conservative hydrophilic amino acids were substituted (N46D, E71Q, and R73H) failed to bind to the asialofetuin agarose, with no sign of retardation. Thus, conservative hydrophilic residues proved to be more important in carbohydrate recognition than the cysteine and tryptophan residues, contrary to the widely accepted concept that these latter residues are essential.

摘要

通过定点诱变研究了人14 kDaβ-半乳糖苷结合凝集素中选定氨基酸残基的作用。制备了10种突变凝集素蛋白,其中每一种中被认为可能与凝集素稳定性相关的残基(6个半胱氨酸残基)之一或脊椎动物β-半乳糖苷结合凝集素家族中高度保守的残基(Asn46、Trp68、Glu71和Arg73)之一被替换。所有半胱氨酸残基之一被丝氨酸取代的突变凝集素(C2S、C16S、C42S、C60S、C88S和C130S)被证明具有与野生型凝集素相当的糖结合能力。此外,发现半胱氨酸2被取代的突变体之一(C2S)在非还原条件下变得相当稳定。在没有β-巯基乙醇的情况下,它保留脱唾液酸胎球蛋白结合活性超过一周,而野生型凝集素在一天内就失去了这种活性。这表明半胱氨酸2的氧化可能是人类14 kDa凝集素失活的关键过程。将高度保守的色氨酸68替换为酪氨酸(W68Y)略微降低了乳糖结合能力,但该突变体仍能强烈吸附在脱唾液酸胎球蛋白琼脂糖上。其他保守亲水性氨基酸被取代的突变凝集素(N46D、E71Q和R73H)未能与脱唾液酸胎球蛋白琼脂糖结合,没有阻滞迹象。因此,与广泛接受的这些后一类残基至关重要的概念相反,保守亲水性残基在碳水化合物识别中被证明比半胱氨酸和色氨酸残基更重要。

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